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Sensitive LC-MS/MS Methods for Amphotericin B Analysis in Cerebrospinal Fluid, Plasma, Plasma Ultrafiltrate, and Urine: Application to Clinical Pharmacokinetics

药代动力学 脑脊液 两性霉素B 尿 色谱法 化学 药理学 血浆 蛋白质沉淀 医学 抗真菌 内科学 生物化学 皮肤病科
作者
Leandro Francisco Pippa,Maria Paula Marques,Anna Christina Tojal da Silva,Fernando Crivelenti Vilar,Tissiana Marques de Haes,Benedito Antônio Lopes da Fonseca,Roberto Martínez,Eduardo Barbosa Coelho,Lauro Wichert‐Ana,Vera Lúcia Lanchote
出处
期刊:Frontiers in Chemistry [Frontiers Media SA]
卷期号:9 被引量:9
标识
DOI:10.3389/fchem.2021.782131
摘要

Neurocryptococcosis, a meningoencephalitis caused by Cryptococcus spp, is treated with amphotericin B (AmB) combined with fluconazole. The integrity of the brain-blood barrier and the composition of the cerebrospinal fluid (CSF) may change due to infectious and/or inflammatory diseases such as neurocryptococcosis allowing for the penetration of AmB into the central nervous system. The present study aimed to develop LC-MS/MS methods capable of quantifying AmB in CSF at any given time of the treatment in addition to plasma, plasma ultrafiltrate, with sensitivity compatible with the low concentrations of AmB reported in the CSF. The methods were successfully validated in the four matrices (25 μl, 5–1,000 ng ml −1 for plasma or urine; 100 μl, 0.625–250 ng ml −1 for plasma ultrafiltrate; 100 μl, 0.1–250 ng ml −1 for CSF) using protein precipitation. The methods were applied to investigate the pharmacokinetics of AmB following infusions of 100 mg every 24 h for 16 days administered as a lipid complex throughout the treatment of a neurocryptococcosis male patient. The methods allowed for a detailed description of the pharmacokinetic parameters in the assessed patient in the beginning (4th day) and end of the treatment with AmB (16th day), with total clearances of 7.21 and 4.25 L h −1 , hepatic clearances of 7.15 and 4.22 L h −1 , volumes of distribution of 302.94 and 206.89 L, and unbound fractions in plasma ranging from 2.26 to 3.25%. AmB was quantified in two CSF samples collected throughout the treatment with concentrations of 12.26 and 18.45 ng ml −1 on the 8th and 15th days of the treatment, respectively. The total concentration of AmB in plasma was 31 and 20 times higher than in CSF. The unbound concentration in plasma accounted for 77 and 44% of the respective concentrations in CSF. In conclusion, the present study described the most complete and sensitive method for AmB analysis in plasma, plasma ultrafiltrate, urine, and CSF applied to a clinical pharmacokinetic study following the administration of the drug as a lipid complex in one patient with neurocryptococcosis. The method can be applied to investigate the pharmacokinetics of AmB in CSF at any given time of the treatment.
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